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About:
Ultrasensitive Monitoring of HIV-1 Viral Load by a Low-Cost Real-Time Reverse Transcription-PCR Assay with Internal Control for the 5′ Long Terminal Repeat Domain
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covidontheweb.inria.fr
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Academic Article
research paper
schema:ScholarlyArticle
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Academic Article
research paper
schema:ScholarlyArticle
isDefinedBy
Covid-on-the-Web dataset
has title
Ultrasensitive Monitoring of HIV-1 Viral Load by a Low-Cost Real-Time Reverse Transcription-PCR Assay with Internal Control for the 5′ Long Terminal Repeat Domain
Creator
Drosten, Christian
Preiser, Wolfgang
Panning, Marcus
Doerr, Hans
Drexler, Jan
Kleber, Luciano
Luna, Souza
Brites, Carlos
Liedigk, Britta
Lippert, Ute
Pedroso, Celia
Samuel, Matthew
Yeats, Jane
Hä, Florian
Stü, Martin
Source
PMC
abstract
Background: Current HIV-1 viral-load assays are too expensive for resource-limited settings. In some countries, monitoring of antiretroviral therapy is now more expensive than treatment itself. In addition, some commercial assays have shown shortcomings in quantifying rare genotypes. Methods: We evaluated real-time reverse transcription-PCR with internal control targeting the conserved long terminal repeat (LTR) domain of HIV-1 on reference panels and patient samples from Brazil (n = 1186), South Africa (n = 130), India (n = 44), and Germany (n = 127). Results: The detection limit was 31.9 IU of HIV-1 RNA/mL of plasma (>95% probability of detection, Probit analysis). The internal control showed inhibition in 3.7% of samples (95% confidence interval, 2.32%–5.9%; n = 454; 40 different runs). Comparative qualitative testing yielded the following: Roche Amplicor vs LTR assay (n = 431 samples), 51.7% vs 65% positives; Amplicor Ultrasensitive vs LTR (n = 133), 81.2% vs 82.7%; BioMerieux NucliSens HIV-1 QT (n = 453), 60.5% vs 65.1%; Bayer Versant 3.0 (n = 433), 57.7% vs 55.4%; total (n = 1450), 59.0% vs 63.8% positives. Intra-/interassay variability at medium and near-negative concentrations was 18%–51%. The quantification range was 50–10 000 000 IU/mL. Viral loads for subtypes A–D, F–J, AE, and AG yielded mean differences of 0.31 log(10) compared with Amplicor in the 10(3)–10(4) IU/mL range. HIV-1 N and O were not detected by Amplicor, but yielded up to 180 180.00 IU/mL in the LTR assay. Viral loads in stored samples from all countries, compared with Amplicor, NucliSens, or Versant, yielded regression line slopes (SD) of 0.9 (0.13) (P <0.001 for all). Conclusions: This method offers all features of commercial assays and covers all relevant genotypes. It could allow general monitoring of antiretroviral therapy in resource-limited settings.
has issue date
2006-07-01
(
xsd:dateTime
)
bibo:doi
10.1373/clinchem.2006.066498
bibo:pmid
16627558
has license
no-cc
sha1sum (hex)
d28a2b8b103901fbcac1df3c927554eae63c32f8
schema:url
https://doi.org/10.1373/clinchem.2006.066498
resource representing a document's title
Ultrasensitive Monitoring of HIV-1 Viral Load by a Low-Cost Real-Time Reverse Transcription-PCR Assay with Internal Control for the 5′ Long Terminal Repeat Domain
has PubMed Central identifier
PMC7108179
has PubMed identifier
16627558
schema:publication
Clin Chem
resource representing a document's body
covid:d28a2b8b103901fbcac1df3c927554eae63c32f8#body_text
is
schema:about
of
named entity 'Brazil'
named entity 'LTR'
named entity 'Long'
named entity 'RUNS'
named entity 'SOUTH AFRICA'
named entity 'HIV-1 RNA'
named entity 'HAVE'
named entity 'REFERENCE'
named entity 'GERMANY'
named entity 'MONITORING'
named entity 'Roche'
named entity 'genotypes'
named entity 'Methods'
named entity 'antiretroviral therapy'
named entity 'evaluated'
named entity 'LTR'
named entity 'confidence interval'
named entity 'assay'
named entity 'internal control'
named entity 'detection limit'
named entity 'South Africa'
named entity 'assay'
named entity 'internal control'
named entity 'LTR'
named entity 'probability of detection'
named entity 'India'
named entity '95% confidence interval'
named entity 'Long Terminal Repeat'
named entity 'Internal Control'
named entity 'Viral Load'
named entity 'Reverse Transcription'
named entity 'real-time PCR'
named entity 'Promega'
named entity 'nucleic acid'
named entity 'HIV-1'
named entity 'Promega'
named entity 'open format'
named entity 'internal control'
named entity 'HIV-1'
named entity 'University of Frankfurt'
named entity 'PCR'
named entity 'Brazil'
named entity 'plasma'
named entity 'transcription'
named entity 'WHO'
named entity 'AVL'
named entity 'WHO'
named entity 'regression analyses'
named entity 'plasma'
named entity 'nucleotide'
named entity 'RNA'
named entity 'hiv-1'
named entity 'molecular methods'
named entity 'milk'
named entity 'Invitrogen'
named entity 'BioMerieux'
named entity 'Germany'
named entity 'virus'
named entity 'fresh-frozen plasma'
named entity 'rhodamine'
named entity 'LTR'
named entity 'Northern Hemisphere'
named entity 'LTR'
named entity 'Clinical Chemistry'
named entity 'nuclease'
named entity 'plasma'
named entity 'pCR'
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